Foxo1 deletion promotes the growth of new lymphatic valves
Joshua P. Scallan, … , Michael J. Davis, Ying Yang
Joshua P. Scallan, … , Michael J. Davis, Ying Yang
Published July 15, 2021
Citation Information: J Clin Invest. 2021;131(14):e142341. https://doi.org/10.1172/JCI142341.
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Research Article Development Vascular biology

Foxo1 deletion promotes the growth of new lymphatic valves

Abstract

Patients with congenital lymphedema suffer from tissue swelling in part due to mutations in genes regulating lymphatic valve development. Lymphatic valve leaflets grow and are maintained throughout life in response to oscillatory shear stress (OSS), which regulates gene transcription in lymphatic endothelial cells (LECs). Here, we identified the first transcription factor, Foxo1, that repressed lymphatic valve formation by inhibiting the expression of valve-forming genes. We showed that both embryonic and postnatal ablation of Foxo1 in LECs induced additional valve formation in postnatal and adult mice in multiple tissues. Our quantitative analyses revealed that after deletion, the total number of valves in the mesentery was significantly (P < 0.01) increased in the Foxo1LEC-KO mice compared with Foxo1fl/fl controls. In addition, our quantitative real-time PCR (RT-PCR) data from cultured LECs showed that many valve-forming genes were significantly (P < 0.01) upregulated upon knockdown of FOXO1. To confirm our findings in vivo, rescue experiments showed that Foxc2+/– mice, a model of lymphedema-distichiasis, had 50% fewer lymphatic valves and that the remaining valves exhibited backleak. Both valve number and function were completely restored to control levels upon Foxo1 deletion. These findings established FOXO1 as a clinically relevant target to stimulate de novo lymphatic valve formation and rescue defective valves in congenital lymphedema.

Authors

Joshua P. Scallan, Luz A. Knauer, Huayan Hou, Jorge A. Castorena-Gonzalez, Michael J. Davis, Ying Yang

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Figure 6

Loss of Foxo1 restores the morphology of valves in Foxc2 heterozygous mice.

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Loss of Foxo1 restores the morphology of valves in Foxc2 heterozygous mi...
(AH) Whole-mount immunostaining of mesenteries collected from P10 control, Foxc2 heterozygotes, Foxc2+/CreERT2 Foxo1+/fl, and Foxc2+/CreERT2 Foxo1fl/fl mice with FOXC2 (red), VE-cadherin (white), PROX1 (green), and ITGA9 (purple). (I) The percentage of Itga9- positive cells from each mesentery. Scale bar is 50 μm in H. Four controls and 4 knockout mesenteries were used in each analysis. All values are mean ± SEM. One-way ANOVA was performed with Tukey’s multiple comparisons test (*P < 0.05, **P < 0.01, ***P < 0.001).